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复制受阻时,人Rad17与增殖细胞核抗原在细胞周期S期晚期的共定位。

Colocalization of human Rad17 and PCNA in late S phase of the cell cycle upon replication block.

作者信息

Dahm Kirsten, Hübscher Ulrich

机构信息

Institute of Veterinary Biochemistry and Molecular Biology, University Zürich-Irchel, Winterthurerstrasse 190, 8057 Zürich, Switzerland.

出版信息

Oncogene. 2002 Oct 31;21(50):7710-9. doi: 10.1038/sj.onc.1205872.

Abstract

In response to replication block or DNA damage in S phase the DNA replication and DNA damage checkpoints are activated. The current model in human predicts, that a Rad17/Replication factor C (RF-C) complex might serve as a recruitment complex for the Rad9/Hus1/Rad1 complex to sites of replication block or DNA damage. In this study we have investigated the fate of the Rad17/RF-C complex after treatment of synchronized Hela cells with the replication inhibitor hydroxyurea. In hydroxyurea treated cells the RF-C p37 subunit became more resistant to extraction. Moreover, co-immunoprecipitation studies with extracts of hydroxyurea treated cells showed an interaction of RF-C p37 with Rad17 and of PCNA with Rad9 and RF-C p37. An enhanced colocalization of Rad17 and PCNA in late S phase after hydroxyurea treatment was observed. Our data suggested, that upon replication block a Rad17/RF-C complex is recruited to sites of DNA lesions in late S phase, binds the Rad9/Hus1/Rad1 complex and enables it to interact with PCNA. An interaction of Rad17/RF-C with PCNA appears to be mediated by the small RF-C p37 subunit, suggesting that PCNA might provide communication between replication checkpoint control and DNA replication and repair.

摘要

在S期,为应对复制阻滞或DNA损伤,DNA复制和DNA损伤检查点被激活。目前人类的模型预测,Rad17/复制因子C(RF-C)复合物可能作为Rad9/Hus1/Rad1复合物被招募至复制阻滞或DNA损伤位点的募集复合物。在本研究中,我们研究了用复制抑制剂羟基脲处理同步化的HeLa细胞后Rad17/RF-C复合物的命运。在羟基脲处理的细胞中,RF-C p37亚基对提取更具抗性。此外,对羟基脲处理细胞提取物的免疫共沉淀研究显示,RF-C p37与Rad17相互作用,PCNA与Rad9和RF-C p37相互作用。观察到羟基脲处理后,在S期末期Rad17和PCNA的共定位增强。我们的数据表明,在复制阻滞时,Rad17/RF-C复合物在S期末期被招募至DNA损伤位点,结合Rad9/Hus1/Rad1复合物,并使其能够与PCNA相互作用。Rad17/RF-C与PCNA的相互作用似乎由小的RF-C p37亚基介导,这表明PCNA可能在复制检查点控制与DNA复制和修复之间提供联系。

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